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Structural and torsional properties of the RAD51-dsDNA nucleoprotein filament

机译:RAD51-dsDNA核蛋白丝的结构和扭转性质

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Human RAD51 is a key protein in the repair of DNA by homologous recombination. Its assembly onto DNA, which induces changes in DNA structure, results in the formation of a nucleoprotein filament that forms the basis of strand exchange. Here, we determine the structural and mechanical properties of RAD51-dsDNA filaments. Our measurements use two recently developed magnetic tweezers assays, freely orbiting magnetic tweezers and magnetic torque tweezers, designed to measure the twist and torque of individual molecules. By directly monitoring changes in DNA twist on RAD51 binding, we determine the unwinding angle per RAD51 monomer to be 45 degrees, in quantitative agreement with that of its bacterial homolog, RecA. Measurements of the torque that is built up when RAD51-dsDNA filaments are twisted show that under conditions that suppress ATP hydrolysis the torsional persistence length of the RAD51-dsDNA filament exceeds that of its RecA counterpart by a factor of three. Examination of the filament's torsional stiffness for different combinations of divalent ions and nucleotide cofactors reveals that the Ca2+ ion, apart from suppressing ATPase activity, plays a key role in increasing the torsional stiffness of the filament. These quantitative measurements of RAD51-imposed DNA distortions and accumulated mechanical stress suggest a finely tuned interplay between chemical and mechanical interactions within the RAD51 nucleoprotein filament.
机译:人RAD51是通过同源重组修复DNA的关键蛋白。它组装到DNA上,诱导DNA结构的变化,导致形成核蛋白丝,形成链交换的基础。在这里,我们确定RAD51-dsDNA细丝的结构和力学性能。我们的测量使用了两个最近开发的磁镊子测定法,即自由旋转的磁镊子和磁扭力镊子,旨在测量单个分子的扭曲和扭力。通过直接监测RAD51结合上DNA扭曲的变化,我们确定每个RAD51单体的退绕角为45度,与其细菌同系物RecA的定量一致。对RAD51-dsDNA细丝扭曲时产生的扭矩的测量结果表明,在抑制ATP水解的条件下,RAD51-dsDNA细丝的扭转持久性长度超过其RecA的扭转持久性长度的三倍。对二价离子和核苷酸辅因子的不同组合检查细丝的抗扭刚度,发现除抑制ATPase活性外,Ca2 +离子在增加细丝的抗扭刚度中起关键作用。这些对RAD51施加的DNA畸变和累积的机械应力的定量测量表明,RAD51核蛋白细丝内化学和机械相互作用之间的相互作用微调。

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